Multilayered blood product

ABSTRACT

A blood product ( 10 ), a method for preparing the blood product, a blood product obtainable by the method and a blood product preparing container means. The blood product comprises components from whole blood, especially fibrin, thrombocytes and leukocytes. The blood product ( 10 ) comprises a first layer ( 21 ), a second layer ( 22 ) and a third layer ( 23 ). The second layer ( 22 ) is adjacent to the first layer ( 21 ) and the third layer ( 23 ). The first layer ( 21 ) defines a first outer surface ( 24 ) of the blood product ( 10 ) and the third layer ( 23 ) defining a second outer surface ( 25 ) of the blood product ( 10 ). The first layer ( 21 ) comprises a majority of fibrin, the second layer ( 22 ) comprises a majority of thrombocytes and the third layer ( 23 ) comprises a majority of leukocytes.

This is a National Phase Application filed under 35 USC 371 ofInternational Application No. PCT/DK2009/050209, filed on Aug. 24, 2009,an application claiming foreign priority benefits under 35 USC 119 ofInternational Application No. PCT/DK2008/000299, filed on Aug. 22, 2008,the content of each of which is hereby incorporated by reference in itsentirety.

TECHNICAL FIELD

The present invention relates to a multilayered blood product, a methodfor preparing the blood product, a blood product obtainable by themethod and a blood product preparing container means.

BACKGROUND ART

The human coagulation system is able to stop bleeding and initiatehealing. The function of the system is well known and extensivelyinvestigated. However, the importance of coagulation products in theinitiation of healing has only been recognized recently.

Blood products, such as fibrin sealants and platelets concentrates, areproduced by isolating the platelet rich plasma (PRP) fromanti-coagulated whole blood. The presence of platelets and plasma partlyimitates the natural human coagulation system upon thrombin activation.This leads to a platelet containing autologous concentrate of growthpromoting factors in a fibrin matrix. Such a composition can be used forcovering wound surfaces and is claimed to initiate healing.

“Platelet-rich fibrin (PRF): A second-generation platelet concentrate.Part I: Technological concepts and evolution, Oral Surg Oral Med OralPathol Oral Radiol Ended 2006; 101:E37-44” by David M. Dohan et aldescribes how to prepare a platelet rich solid fibrin network from wholeblood without adding any additives or reagents. The PRF protocol is: Ablood sample is taken without anticoagulant in 10-mL glass tubes orglass coated plastic which are immediately centrifuged at approximately400 g for 10 minutes. The absence of anticoagulant implies theactivation in a few minutes of most platelets of the blood sample incontact with the glass tube walls and the release of the coagulationcascades. Fibrinogen is initially concentrated in the top part of thetube, before the circulating thrombin transforms it into fibrin. Afibrin clot is then obtained in the middle of the tube, extending fromthe upper part of the red corpuscles at the bottom of the tube to thecellular plasma at the top. Platelets are trapped massively in thefibrin meshes. The success of this technique entirely depends on thespeed of blood collection and transfer to the centrifuge. Indeed,without anticoagulant, the blood samples start to coagulate almostimmediately upon contact with the tube glass, and it takes a minimum ofa few minutes of centrifugation to concentrate fibrinogen in the middleand upper part of the tube. Quick handling is the only way to obtain aclinically usable PRF clot. If the duration required to collect bloodand launch centrifugation is overly long, failure will occur: The fibrinwill polymerize in a diffuse way in the tube and only a small blood clotwithout consistency will be obtained. In conclusion, the PRF protocolmakes it possible to collect a fibrin clot charged with serum andplatelets. By removing the clot from the tube, manually cutting of thered cells part, and manually driving out the fluids trapped in thefibrin matrix (serum), practitioners will obtain autologous fibrinmembranes.

However this fibrin network includes a red thrombus containing asubstantial part of red blood cells, which have to be manually cut off.Furthermore the components of the produced fibrin network, such asfibrin, leukocytes and thrombocytes, are arbitrary distributed andenmeshed within the product. The recovery of leukocytes are notdescribed and at the low g force used, the recovery of leukocytes is lowas some will be located in the red cell part. The enmeshment of cellswithin the fibrin leads to absent or slow release of these cells andthereby inhibits the contact-dependent anti-microbicidal potential ofthe included leucocytes.

“Oral Surg Oral Med Oral Pathol Oral Radial Endod 2006; 101:E37-44 and2006; 101:E45-50” by Dohan et al describes a network that does notrepresent a platelet concentrate in a shape and structure, which isdirectly applicable for covering wound surfaces. To obtain a shape andform/rigidity useable for covering wound surfaces and prevent red bloodcell inclusion, the known platelet rich solid fibrin network will haveto be reshaped manually and compressed. Furthermore, the methodcomprises several steps and cannot be prepared in one closed system andis therefore not convenient for clinical use.

“Cell separation in the buffy coat. Biorheology. 1988; 25 (4):663-73” bySutton et al describes how anti-coagulated full blood will separate intoseveral layers upon centrifugation or passive sedimentation; Red bloodcells, leukocytes and platelets (=buffycoat) and plasma. Further, byusing centrifugation force of 10000 g for 10 minutes and using a floatof density of 1.053, the buffy coat can be fixed by Glutaraldehyde, andremoved for investigation; however, this cannot be used clinically dueto the toxicity of the Glutaraldehyde. Several methods for extractingthe buffycoat from anti-coagulated blood exists including the use ofdensity defined substances (ie. Lymphoprep). In addition to the need foranti-coagulated blood the extracted cells will be suspended—and mixed(disorganized)—in the plasma that inevitably will be included.

EP 1637145A describes a method of filtration of cells from a suspension(eg. blood cells including platelets and leukocytes) through a sheetlike porous membrane, leaving the cells in the membrane as described.The sheet porous material can be prepared from fibrin. However, nolayered structure is obtained, the cell are trapped in depth in theporous material and the use of allogeneic fibrin raises the risk ofcross infection from other humans. Furthermore, the method comprisesseveral steps and cannot be prepared in one closed system and istherefore not convenient for clinical use.

Known methods are limited in their use, especially clinical use. Theaddition of anti-coagulants prior to cell separation lead to productsnot completely autologous, furthermore the release of substancespromoting wound healing (e.g. growth factors) requires mixing with othernon-autologous substances (e.g. thrombin, Ca₂ ⁺ etc.) leading tohomogenous final products without the desired distribution of cells.

Known methods excluding anti-coagulation lead to a disorganizeddistribution of cells, the cells are locked inside the product,effectively limiting the release and potential of these cells.Furthermore these methods need manual handling outside a closed systemto obtain a product physically suitable for clinical use, aninadequately defined handling that leads to a variable outcome with alower than optimal cell yield. Furthermore, the manual handling willrequire labor time (cost) and prolong the preparation time.

Methods describing a well defined layered structure depend onanti-coagulation and addition of toxic components, not suitable forclinical use, for the fixation and self-sustainability of the structureobtained.

DISCLOSURE OF INVENTION

The object of the invention is to provide a new and improved bloodproduct which overcomes or ameliorates at least one of the disadvantagesof the prior art or which provides a useful alternative. The object ofthe invention is furthermore to provide a new and improved method forobtaining the blood product which overcomes or ameliorates at least oneof the disadvantages of the prior art or which provides a usefulalternative.

The object of the invention is obtained by a blood product comprisingcomponents from whole blood, especially fibrin, thrombocytes andleukocytes, the blood product comprising a first layer, a second layerand a third layer, the second layer being adjacent to the first layerand the third layer, the first layer defining a first outer surface ofthe blood product and the third layer defining a second outer surface ofthe blood product, the first layer comprising a majority of fibrin, thesecond layer comprising a majority of thrombocytes and the third layercomprising a majority of leukocytes. Hereby, a blood product with amultilayered structure is provided, each layer provides differentfunctionality due to different composition of each of the layers. Theblood product is self-supporting, compact and solid, and the bloodproduct has a structure, such that the blood product is directlyapplicable for the intended use. By majority is meant, that a component,such as fibrin, thrombocytes or leukocytes, comprises at least 50%, 55%,60%, 65%, 70%, 75%, 80%, 85%, 90%, 95%, 98%, 99% or even 100%, or anyinterval that can be defined from combinations of these mentionedpercentages, volume—and/or mass wise of the respective layer and/orvolume- and/or mass wise of the blood product. The first, the second andthe third layer are each continuous and/or substantially parallel toeach other, e.g. forming a stratified and/or multilayered blood product.The blood product preferably consists of three layers, e.g. a firstlayer comprising a majority of fibrin, a second layer comprising amajority of thrombocytes and a third layer comprising a majority ofleukocytes. The blood product has preferably a maximumwidth/thickness-ratio of 1, 2, 3, 4 or 5, however the ratio may be up to10, 15, 20, 25, 30, 40, 50, 60, 70, 80, 90 or even up to 100, where thewidth is measured along the layers of the blood product and thethickness is measured perpendicular to the layers of the blood product.

In another aspect of the invention, the blood product solely consists ofcomponents from whole blood. Hereby, a blood product is provided thatsolely consists of components from whole blood, meaning that noadditives are added to the whole blood and/or the blood product, andthat the blood product is directly derivable from whole blood, fractionsof whole blood or combinations of fractions of whole blood.

In another aspect of the invention, the blood product is autologous.

In another aspect of the invention, the blood product is flexible.Hereby, a blood product is provided that can withstand applied stressduring normal use without rupturing. Due to the flexibility of the bloodproduct, the blood product conforms most continuous contours whereto theblood product is applied.

In another aspect of the invention, the blood product further comprisesa first substance chosen from a group comprising fibroblasts,keratinocyte cells and hyaluronic acid. Hereby, a blood product isprovided which includes additional cells known to be important for skinregeneration and thereby further improves the healing potential ofchronic wounds, especially wounds in areas with low or unviable adjacenttissue. Hyaluronic acid, a known component of skin, has the potential toincrease the water binding capacity of the blood product as well asincrease the potential for incorporation/infiltration of the bloodproduct in areas of tissue loss.

The invention also relates to, a blood product for therapeutic useand/or use of a blood product according to the aforementioned fortherapeutic use.

The invention also relates to use of a blood product for manufacturingof a medicament for therapeutic use.

The invention also relates to a blood product for treatment of a woundand/or use of a blood product according to the aforementioned fortreatment of a wound.

The invention also relates to use of a blood product for manufacturingof a medicament for treatment of a wound. Hereby, a blood product isprovided which is particular suitable for manufacturing of a medicamentfor treatment of a wound. By applying the second outer surface definedby the third layer against the wound, the wound is kept and/ormaintained substantially sterile, e.g. free of infection, as the thirdlayer comprises a majority of leukocytes, which are the first activecells and thus controls infection and attracts other cells includingmacrophages, while the second layer comprises a majority of thrombocyteswhich comprises growth promoting factors that stimulates the fibroblastcells, while the first layer of the blood product comprises a majorityof fibrin, and thus the first outer surface of the blood productprovides an effective protection against contamination from thesurroundings; the first layer furthermore comprises growth promotingfactors, which is released over time. By applying the second outersurface defined by the third layer against the wound, the wound is keptand/or maintained substantially free of infection, as the third layercomprises a majority of leukocytes which are easily released from theproduct, Leukocytes are cells of the immune system defending the bodyagainst infection and foreign bodies, thus they control infection andfurther attracts other cells including macrophages. The second layercomprises a majority of thrombocytes which comprises growth promotingfactors that stimulates the cells. As the leukocytes quickly will bereleased from the product, the second layer will face the wound surfacefor optimal delivery of growth promoting substances to the wound. Thefirst layer of the blood product comprises a majority of fibrin, andthus the first outer surface of the blood product provides an effectiveprotection against contamination from the surroundings; the first layerfurthermore comprises growth promoting factors, which is released overtime.

The invention also relates to a blood product for autologous use and/oruse of a blood product, for autologous use generally having componentsfrom whole Mood, especially fibrin, thrombocytes and leukocytes, theblood product (10) comprising a first layer (21). a second layer (22)and a third layer (23).

The invention also relates to use of a blood product for manufacturingof an autologous medicament.

The invention also relates to a blood product for surgical use, e.g. toseal of an area, to prevent post surgical adherence and/or use inanastomosis procedures and/or use of a blood product according to theaforementioned for surgical use.

The invention also relates to use of a blood product or manufacturing ofa medicament for surgical use.

In another aspect of the invention, the blood product is foranastomosis. Use of a blood product obtainable by a method according tothe aforementioned for anastomosis.

In another aspect of the invention, the blood product is used formanufacturing of a medicament for anastomosis.

The invention relates also to a method for preparing a blood productfrom a volume of whole blood, the method comprising the following steps:a) placing the volume of whole blood in a container means, the containermeans comprising a first material defining an inner surface in which thewhole blood is in contact with, b) activating coagulation of the wholeblood, c) separating the whole blood into erythrocytes, serum and bloodproduct by a centrifugal force acting on the whole blood placed in thecontainer means, whereby the whole blood separates into layerscomprising erythrocytes, blood product and serum due to the differencesin densities between the erythrocytes, blood product and serum, theblood product comprising fibrin, leukocytes and thrombocytes, theapplied centrifugal force being at least 1000 times greater than thegravity force, e.g. g, acting on the whole blood, the centrifugal forcevarying inversely with the time of the centrifugation, and d) removingthe blood product from the container means. Hereby, a method is providedwhereby a blood product is derivable from whole blood. The method can beprocessed in one cycle in a closed system, since there is no need for anisolation of the erythrocytes; however the method can also be performedusing an isolation of the erythrocytes.

The yield of the method for extracting fibrin from the whole blood is atleast above 10%, 20%, 30%, 40%, 50%, 60%, 70%, 80%, 90%, 95%, 97%, 98%,99% or even 100%, while the yield of the method for extractingleukocytes from the whole blood is at least above 10%, 20%, 30%, 40%,50%, 60%, 70%, 80%, 90%, 95%, 97%, 98%, 99% or even 100%, while theyield of the method for extracting thrombocytes from the whole blood isat least above 10%, 20%, 30%, 40%, 50%, 60%, 70%, 80%, 90%, 95%, 97%,98%, 99% or even 100%. The obtainable blood product has a volume lessthan 30%, 20%, 15%, 10% or even less than 5% of the volume of the wholeblood. Hereby, a method is provided whereby a blood product isobtainable by e.g. centrifugation giving rise to a centrifugal force.The applied centrifugal force is at least 1000, 2000, 3000, 4000, 5000,6000, 7000, 8000, 9000, 10000, 11000, 12000, 13000, 14000, 15000, 16000,17000, 18000, 19000 or even 20000 times greater than the gravity force,e.g. g, acting on the whole blood, or the applied centrifugal force iswithin any interval that can be defined from combinations of thementioned numbers. The centrifugal force is applied for at least 30seconds, 40 seconds, 50 seconds, 60 seconds, 1 minute, 2 minutes, 3minutes, 4 minutes, 5 minutes, 6 minutes, 7 minutes, 8 minutes, 9minutes, 10 minutes, 11 minutes, 12 minutes, 13 minutes, 14 minutes, 15minutes, 16 minutes, 17 minutes, 18 minutes, 19 minutes, 20 minutes, 21minutes, 22 minutes, 23 minutes, 24 minutes, 25 minutes, 26 minutes, 27minutes, 28 minutes, 29 minutes or 30 minutes, or the centrifugal forceis applied within any interval that can be defined from combinations ofthe mentioned numbers.

In one aspect of the invention, the yield of the method for extractingfibrin from the whole blood is at least above 60%.

In one aspect of the invention, the yield of the method for extractingleukocytes from the whole blood is at least above 50%.

In one aspect of the invention, the yield of the method for extractingthrombocytes from the whole blood is at least above 60%.

In one aspect of the invention, the centrifugal force is applied for atleast 30 seconds.

In one aspect of the invention, the blood product solely consists ofcomponents from whole blood. Hereby, a method is provided whereby ablood product is derivable from whole blood, thus solely consisting ofcomponents from whole blood. Thus the method is performed without addingany additives to the whole blood and/or the blood product.

In another aspect of the invention, the coagulation in step b) isactivated by the first material defining the inner surface. Hereby, amethod is provided in which the coagulation is initiated when the wholeblood is brought in contact with the inner surface, thus it can beavoided to add any object or the like to the whole blood to initiatecoagulation.

In another aspect of the invention, the coagulation in step b) isactivated by exposing the whole blood to an object, such as a glassbead. Hereby, a method is provided in which the coagulation is initiatedwhen the whole blood is brought in contact with the object added to thewhole blood. Hereby, the coagulation can be initiated at a chosen pointof time, which is optimal for the method.

In another aspect of the invention, the first material of the innersurface of the container means is chosen from a group comprising ofpolypropylene, polyethylene, polycarbonate, polyamide, acrylonitrilebutadiene styrene, styrene, modified styrene, polyurethane and otherpolymer materials. The polymers in the mentioned group can furthermorebe glass-filled. Hereby, a method is provided where a container meanswith an inner surface of a first material can be typical test tubes orthe like made from all kinds of polymers, metal or glass. The materialcan also be chosen so the material property pro vides a minimal adhesiveforce/friction between the blood product and the inner surface.Polyamide and polyurethane are preferred as these materials initiatescoagulation within a preferred level of activation which is higher thanthe level obtained using other polymers.

In another aspect of the invention, the inner surface of the containermeans is surface treated, e.g. coated, in order to lower frictionbetween the blood product and the inner surface of the first material.Hereby, a method is provided where a container means with an innersurface of a first material can be typical test tubes or the like madefrom all kinds of polymers, metal or glass. The inner surface can besurface treated and/or coated to obtain a minimal adhesiveforce/friction between the blood product and the inner surface.

In another aspect of the invention, the centrifugal force is greaterthan an adhesive force acting between the inner surface and the bloodproduct. Hereby, a method is provided where the centrifugal force isdominant as compared to the adhesive force, which secures a well definedlayered structure of the blood product. The centrifugal force can be atleast 10, 100, 1000, 5000, 10000, 20000, 50000, 100000, 1000000 or even10000000 times greater than the adhesive force, or the centrifugal forceis within any interval that can be defined from combinations of thementioned numbers. In another aspect of the invention, the centrifugalforce and centrifugation time is of such strength that the adhesiveforce acting between the inner surface and the fibrin is broken/releasedand thereby allowing the fibrin layer to be compacted/compressed.Hereby, a method is provided where the centrifugal force is dominant ascompared to the adhesive force, which secures a well defined layeredstructure of the blood product. The centrifugal force needed to releasethe adhesion to the wall will depend on the fibrin density. The fibrindensity will depend on several factors including coagulation activation,fibrin concentration, time, etc. The centrifugation force can be atleast 10, 100, 1000, 5000, 10000, 20000, 50000, or even 100000, g, orthe centrifugal force is within any interval that can be defined fromcombinations of the mentioned numbers.

In another aspect of the invention, the blood product adhering to theinner surface is detached from the inner surface, at least once, duringstep c). Hereby, a method is provided where the possible adhesion of theblood product to the inner surface can be dealt with by separating theblood product at least once during step c). The separation can be doneby mechanical means such as by cutting or the like. The compacting ofthe fibrin can then be performed at lower g-force as the g-force doesnot need to release the fibrin from the wall.

In another aspect of the invention, the method further comprises acompacting step, where the blood product is compacted by a compactingmeans, such as a filter placed in the container means. Hereby, a methodis provided where the blood product can be compacted by e.g. a filter.The filter can be placed fixed or movable in the container means and thefilter can be used to isolate the blood product.

In another aspect of the invention, the method further comprises anisolation step, where the erythrocytes are isolated from the bloodproduct during step c). Hereby, a method is provided where theerythrocytes are isolated from the serum and the blood product duringthe method.

In another aspect of the invention, the method further comprises awashing step where the blood product is washed, so substantially allerythrocytes and/or serum attached to the blood product are detached.Hereby, a method is provided so the blood product is substantially cleanfrom other components, that of the blood product itself. The serumformed during the centrifugation may be used as a washing fluid.

In another aspect of the invention, the container means is a tubecomprising an open end, closable by a detachable lid, and a closed end.Hereby, a method is provided where a standard test tube or the like canbe used to perform the method.

In another aspect of the invention, step b) precedes step a). Hereby,the coagulation can be activated before the whole blood is placed in thecontainer means, thus the container means does not need to comprise anycoagulation activator and/or the whole blood does not need to comprise acoagulation activator when the whole blood is placed in the containermeans. The coagulation can as an example, be activated during blooddrawing by placing glass beads in the blood drawing tubing, or choosinga tubing material that will activate blood. Thus it can be avoided toadd any object or the like to the whole blood to initiate coagulation.

In another aspect of the invention, step b) occurs at least 1 minutesbefore step a). Hereby a method is provided where very fast handling isnot necessary. Step b) can occur at least 30 seconds, 40 seconds, 50seconds, 60 seconds, 1 minute, 2 minutes, 3 minutes, 4 minutes, 5minutes, 6 minutes, 7 minutes, 8 minutes, 9 minutes, 10 minutes, 11minutes, 12 minutes, 13 minutes, 14 minutes, 15 minutes, 16 minutes, 17minutes, 18 minutes, 19 minutes or even 20 minutes before step a). Thelevel of activation of coagulation in step b) can also be controlled bythe method. This allows the time between step b) and a) to be prolongedas the cell separation in step c) has to occur before fibrin levels issufficient to inhibit cell separation.

In another aspect of the invention, step b) occurs concurrently withstep c). Hereby, the coagulation can be activated at an optimum point oftime for the method during step c).

The coagulation can be activated/initiated by a coagulation activatorintegrated into the container means, and/or by using a containermaterial that will activate the blood. The coagulator material can be anobject, such as glass beads, added to the whole blood in the containermeans.

In another aspect of the invention, a first substance chosen from agroup comprising fibroblasts, keratinocyte cells and hyaluronic acid isadded to the whole blood. Hereby, a blood product is obtainable whichincludes additional cells known to be important for skin regenerationand thereby further improves the healing of chronic wounds, especiallywounds in areas with low or unviable adjacent tissue. Hyaluronic acid, aknown component of skin, has the potential to increase the water bindingcapacity of the blood product as well as increase the potential forincorporation/infiltration of the blood product in areas of tissue loss.

In another aspect of the invention, the compacting means, such as afilter, has a first fixed position and a second position. The filter isfixed in a position in the part of the container means containing theerythrocytes during the first part of the centrifugation where theleukocytes and thrombocytes has been separated, while the fibrin in theserum has not been compacted. Provided that the density of the filter isless than that of serum, a release of the filter will cause the filterto be transferred to the top of the tube and thereby collecting theleucocyte and thrombocyte layer and compacting the fibrin layer.

In another aspect of the invention, the compacting means, such as afilter, is fixed in the first fixed position by a deformation in thecontainer means wall. The filter is fixed by deforming the tube wall.The filter is released by removing the deformation of the wall.

In another aspect of the invention, plasma comprising fibrin and a buffycoat comprising leukocytes and thrombocytes are used instead of wholeblood. Hereby, a method is provided where whole blood excludingerythrocytes can be used, thus the blood product is directly derivablefrom whole blood, fractions of whole blood or combinations of fractionsof whole blood.

In another aspect of the invention, the method is performed within 15minutes. The method is performed within at least 1 minute, 2 minutes, 3minutes, 4 minutes, 5 minutes, 6 minutes, 7 minutes, 8 minutes, 9minutes, 10 minutes, 11 minutes, 12 minutes, 13 minutes, 14 minutes, 15minutes, 16 minutes, 17 minutes, 18 minutes, 19 minutes, 20 minutes, 21minutes, 22 minutes, 23 minutes, 24 minutes, 25 minutes, 26 minutes, 27minutes, 28 minutes, 29 minutes or at least 30 minutes.

In another aspect of the invention, the blood product obtained by themethod is the blood product generally having components from wholeblood, especially fibrin, thrombocytes and leukocytes, the blood product(10) comprising a first layer (21). a second layer (22) and a thirdlayer (23).

The invention also relates to a blood product obtainable by a methodcomprising components from whole blood, especially fibrin, thrombocytesand leukocytes, the blood product comprising a first layer, a secondlayer and a third layer, the second layer being adjacent to the firstlayer and the third layer, the first layer defining a first outersurface of the blood product and the third layer defining a second outersurface of the blood product, the first layer comprising a majority offibrin, the second layer comprising a majority of thrombocytes and thethird layer comprising a majority of leukocytes. Hereby, a blood productis obtainable with a multilayered structure; where each of the layersprovides different functionality due to each layers differentcomposition. The blood product is self-supporting, compact and solid,and the blood product has a structure, such that the blood product isdirectly applicable for the intended use. By majority is meant, that acomponent, such as fibrin, thrombocytes or leukocytes, comprises atleast 50%, 55%, 60%, 65%, 70%, 75%, 80%, 85%, 90%, 95%, 98%, 99% or even100%, or any interval that can be defined from combinations of thesementioned percentages, volume- and/or mass wise of the respective layeror volume- and/or mass wise of the blood product. The first, the secondand the third layer are each continuous and/or substantially parallel toeach other, e.g. forming a stratified and/or multilayered blood product.The blood product preferably consists of three layers, e.g. a firstlayer comprising a majority of fibrin, a second layer comprising amajority of thrombocytes and a third layer comprising a majority ofleukocytes. The blood product has preferably a maximumwidth/thickness-ratio of 1, 2, 3, 4 or 5, however the ratio may be up to10, 15, 20, 25, 30, 40, 50, 60, 70, 80, 90 or even up to 100, where thewidth is measured along the layers of the blood product and thethickness is measured perpendicular to the layers of the blood product.

In another aspect of the invention, a majority of the fibrin comprisedin the blood product is comprised in the first layer. Hereby, a bloodproduct is obtainable where a majority of the fibrin comprised in theentire blood product is comprised in the first layer.

In another aspect of the invention, a majority of the thrombocytescomprised in the blood product is comprised in the second layer. Hereby,a blood product is obtainable where a majority of the thrombocytescomprised in the entire blood product is comprised in the second layer.

In another aspect of the invention, a majority of the leukocytescomprised in the blood product is comprised in the third layer. Hereby,a blood product is obtainable where a majority of the leukocytescomprised in the entire blood product is comprised in the third layer.

In another aspect of the invention, the blood product solely consists ofcomponents from whole blood. Hereby, a blood product is obtainable thatsolely consists of components from whole blood, meaning that noadditives are added to the whole blood and/or the blood product, and theblood product is directly derivable from whole blood, fractions of wholeblood or combinations of fractions of whole blood.

In another aspect of the invention, the blood product is autologous.

In another aspect of the invention, the blood product is flexible.Hereby, a blood product is obtainable that can withstand applied stressduring normal use without rupturing. Due to the flexibility of the bloodproduct, the blood product conforms most continuous contours whereto theblood product is applied.

In another aspect of the invention, the blood product further comprisesa first substance chosen from a group comprising fibroblasts,keratinocyte cells and hyaluronic acid. Hereby, a blood product includesadditional cells known to be important for skin regeneration and therebyfurther improves the healing of chronic wounds, especially wounds inareas with low or unviable adjacent tissue. Hyaluronic acid, a knowncomponent of skin, has the potential to increase the water bindingcapacity of the blood product as well as increase the potential forincorporation/infiltration of the blood product in areas of tissue loss.

In another aspect of the invention, the blood product is for therapeuticuse. Use of a blood product obtainable by a method according to theaforementioned for therapeutic use.

In another aspect of the invention, the blood product is used formanufacturing of a medicament for therapeutic use.

In another aspect of the invention, the blood product is for treatmentof a wound. Use of a blood product obtainable by a method according tothe aforementioned for treatment of a wound.

In another aspect of the invention, the blood product is used formanufacturing of a medicament for treatment of a wound. Hereby, a bloodproduct is obtainable which is particular suitable for manufacturing ofa medicament for treatment of a wound. By applying the second outersurface defined by the third layer against the wound, the wound is keptand/or maintained substantially sterile, e.g. free of infection, as thethird layer comprises a majority of leukocytes, which are the firstactive cells and thus controls infection and attracts other cellsincluding macrophages, while the second layer comprises a majority ofthrombocytes which comprises growth promoting factors that stimulateswound healing and/or granulation, while the first layer of the bloodproduct comprises a majority of fibrin, and thus the first outer surfaceof the blood product provides an effective protection againstcontamination from the surroundings; the first layer furthermorecomprises growth promoting factors, which is released over time. Byapplying the second outer surface defined by the third layer against thewound, the wound is kept and/or maintained substantially free ofinfection, as the third layer comprises a majority of leukocytes whichare easily released from the product. Leukocytes are cells of the immunesystem defending the body against infection and foreign bodies, thusthey control infection and further attracts other cells includingmacrophages. The second layer comprises a majority of thrombocytes whichcomprises growth promoting factors that stimulates the cells. As theleukocytes quickly will be released from the product, the second layerwill face the wound surface for optimal delivery of growth promotingsubstances to the wound. The first layer of the blood product comprisesa majority of fibrin, and thus the first outer surface of the bloodproduct provides an effective protection against contamination from thesurroundings; the first layer furthermore comprises growth promotingfactors, which is released over time.

In another aspect of the invention, the blood product is used forautologous use. Use of a blood product obtainable by a method accordingto the aforementioned for autologous use.

In another aspect of the invention, the blood product is used formanufacturing of an autologous medicament.

The invention also relates to a blood product for surgical use, e.g. toseal of an area, to prevent post surgical adherence and/or use inanastomosis procedures and/or use of a blood product according to theaforementioned for surgical use.

In another aspect of the invention, the blood product is foranastomosis. Use of a blood product obtainable by a method according tothe aforementioned for anastomosis.

In another aspect of the invention, the blood product is used formanufacturing of a medicament for anastomosis.

The invention also relates to a blood product preparing container meansfor preparing a blood product generally having components from wholeblood, especially fibrin, thrombocytes and leukocytes, the blood product(10) comprising a first layer (21). a second layer (22) and a thirdlayer (23). wherein the blood product preparing container meanscomprises potyamide and/or poryurethane Hereby, a blood productpreparing container means is provided which activates the coagulation ofwhole blood, or more specific provides a complement activation, and atthe same time comprises a polymer material, which is preferred overglass containers, due to the polymers fragility and/or costs, and otherpolymer containers due to their coagulation-inactive properties. Thefact that pofyamide and/or potyurethane activates the coagulation ofwhole blood is surprising and provides a better alternative to thetypical known glass container means and coagulation-inactive polymercontainer means, as the blood product preparing container means combinesthe advantages of the known glass container means and porymer containermeans.

The invention also relates to use of a blood product preparing containermeans as described herein for manufacturing of a blood product generallyhaving components from whole blood, especially fibrin, thrombocytes andleukocytes, the blood product (10) comprising a first layer (21), asecond layer (22) and a third layer (23).

The invention also relates to a blood product preparing container means,wherein the blood product preparing container means comprises polyamideand/or polyurethane. Hereby, a blood product preparing container meansis provided which activates the coagulation of whole blood, or morespecific provides a complement activation, and at the same timecomprises a polymer material, which is preferred over glass containers,due to the polymers fragility and/or costs, and other polymer containersdue to their coagulation-inactive properties. The fact that polyamideand/or polyurethane activates the coagulation of whole blood issurprising and provides a better alternative to the typical known glasscontainer means and coagulation-inactive polymer container means, as theblood product preparing container means combines the advantages of theknown glass container means and polymer container means.

The invention also relates to use of a blood product preparing containermeans wherein the blood product preparing container means comprisespolvamide and/or potvurethane for manufacturing of a blood product.

BRIEF DESCRIPTION OF THE DRAWING

The invention is explained in detail below with reference to thedrawing, in which

FIG. 1 shows a cross sectional view of a first embodiment of thecontainer means according to the invention,

FIG. 2 shows a cross sectional view of a second embodiment of thecontainer means according to the invention,

FIG. 3 shows a cross sectional view of a third embodiment of thecontainer means according to the invention,

FIG. 4 shows a cross sectional view of a fourth embodiment of thecontainer means according to the invention,

FIG. 5 shows a cross sectional view of the first embodiment of thecontainer means according to the invention,

FIG. 6 shows a cross sectional view of the second embodiment of thecontainer means according to the invention,

FIG. 7 shows a cross sectional view of the third embodiment of thecontainer means according to the invention,

FIG. 8 shows a cross sectional view of the fourth embodiment of thecontainer means according to the invention,

FIG. 9 illustrates a cross sectional view of an embodiment of the bloodproduct according to the invention, and

FIG. 10 shows a cross sectional view of an embodiment of the bloodproduct according to the invention.

DETAILED DESCRIPTION

FIGS. 1 to 4 illustrates respectively a first, second, third and fourthembodiment of a container means 1. The container means 1 in the fourembodiments comprises a cavity having an inner surface 3. The cavitybeing defined by a wall 4, a closed end 12 and an open end closeable bya lid 2. The container means 1 defines a volume of whole blood 5 and isclosed to the surroundings via the lid 2 mounted on the open end of thecontainer means 1. The container means 1 can be made of any material,and the material can be chosen, so that the material of the containermeans 1 due to contact with the whole blood 5 via the inner surface 3activates the coagulation cascade of the whole blood 5, which is thecase for the first embodiment in FIG. 1 and the third embodiment in FIG.3. Alternatively, the material of the container means 1 can be chosen sothat the material is inactive in relation to the whole bloods 5coagulation cascade, which is the case for the second embodiment in FIG.2 and the fourth embodiment in FIG. 3, where an object 7, made of amaterial that activates the bloods 5 coagulation cascade, instead isadded to the whole blood 5, such that the object 7 is used to activatethe whole bloods 5 coagulation cascade. The inner surface 3 of thecontainer means 1 in the four embodiments can be coated and/or surfacetreated in order to lower the friction between the inner surface 3 andany components of the blood 5. Furthermore the material of the containermeans 1 can be chosen, so that a low friction between the inner surface3 and any component of the blood 5 is obtained, e.g. by choosing amaterial with a low protein binding capacity. In the third and fourthembodiment shown in FIGS. 3 and 4 a compaction means 8, such as afilter, is placed in the container means 1, whereby the blood product 10is compacted against the compaction means.

The compacting means 8 can be locked in the closed end 12 of thecontainer means 1, where the erythrocytes are located, in the initialpart of the process. At a later point in time the compacting means 8 canbe released and provided that the density of the compacting means 8 islower that the plasma, the compacting means will be forced to the top ofthe plasma. By removing the lid 2, the blood product 10 can be removedfrom the container means 1. The compaction means 8, or part of thecompacting means, can be used to support the blood product 10 duringtransport from the container means 1.

The whole blood 5 in all four embodiments are subjected to a centrifugalforce 6 acting downwards as illustrated, however the centrifugal force 6is not limited to act in the shown direction. The centrifugal force 6functions as a separation means, since the components of the whole blood5 have different densities and thus will respond differently to thecentrifugal force 6.

FIGS. 1 to 4 illustrates the four embodiments of the container means 1at a point of time where the centrifugal force 6 just been applied,hence no separation of the whole blood 5 is visible, while FIGS. 5 to 8respectively shows the first, second, third and fourth embodiment of thecontainer means 1 at a point of time where the centrifugal force 6 hasbeen acting sufficiently long and with sufficiently magnitude, hence thewhole blood 5 has separated into serum 9, with the fibrin distributedthrough this serum part, platelets and leucocytes layer 10 anderythrocytes 11. At a later point in time the compacting means 8 can bereleased and provided that the density of the compacting means 8 islower than that of the serum, the compacting means will be forced to thetop of the serum and thereby releasing the fibrin from the wall andcompacting the fibrin. By removing the lid 2, the blood product 10 canbe removed from the container means 1. The compaction means 8, or partof the compacting means, can be used to support the blood product 10during transport from the container means 1.

FIG. 9 illustrates a schematic cross sectional view of the blood product10 comprising a first layer 21, a second layer 22 and a third layer 23,where the second layer is adjacent to the first layer 21 and the thirdlayer 23. The first layer 21 defines a first outer surface 24 of theblood product 10 and the third layer 23 defines a second outer surfaceof the blood product 10. The first layer 21 comprises a majority offibrin, while the second layer 22 comprises a majority of thrombocytesand the third layer 23 comprises a majority of leukocytes. Thus theblood product 10 has a well defined multilayer structure with each layerhaving different compositions and therefore having differentfunctionalities.

FIG. 10 shows a cross sectional view of a blood product obtainedexperimentally by using a test tube made of polypropylene as containermeans.

The invention has been described with reference to a preferredembodiment. However, the scope of the invention is not limited to theillustrated embodiment, and alterations, combinations and modificationscan be carried out without deviating from the scope of the invention.

EXAMPLES Example 1

-   -   1. Take a plastic container (eg. a 2 ml microcentrifuge tube)        and add a coagulation trigger, eg. 4 glass beads (diameter 2 mm)    -   2. Draw blood into the plastic container.    -   3. Mix the blood and coagulation activator end-over-end for 2        min.    -   4. Spin the container at 16200 g for 20 min.    -   5. After this the blood product will be formed in a layer        between the red blood cells and the serum.    -   6. Remove the blood product using forceps.

In this method the needed spin time and spin speed will depend on thepower of activation. E.g. if the coagulation activation is high, thecells must be separated before they are trapped in the fibrin network,this will require a high spin speed. Due to the high spin speed, spintime can be low.

Example 2

-   -   1. Take a standard 50 ml centrifugation tube container and ad a        coagulation trigger, eg. glass beads.    -   2. Draw blood into the centrifugation tube.    -   3. Mix the blood in the tube for 1 min.    -   4. Spin the tube at 3000 g for 20 min    -   5. Open the lid and loosen the fibrin (formed in the serum in        the top part) from the wall (using a thin plastic stick or        needle)    -   6. Spin the sample another 5 min at 3000 g.    -   7. After this the blood product will be formed in a layer        between the red cell and serum.    -   8. Remove the blood product using forceps

Example 3

-   -   1. Take a 20 ml container (inner diameter: 26 mm) prepared out        of polyamide or polyurethane    -   2. Ad a lid and create a vacuum inside the container    -   3. Insert a needle in the patient    -   4. Connect the needle to the container without losing the vacuum    -   5. Draw blood into the plastic container by the help of the        vacuum.    -   6. Spin the tube at 15000 g for 12 min    -   7. After this the blood product will be formed in a layer        between the red cell and serum.    -   8. Remove lid and remove the blood product with for forceps

Example 4

-   -   1. Take a 20 ml container (inner diameter: 26 mm) prepared out        of polyamide or polyurethane    -   2. Place a disk in the bottom of the container. The density of        the disk shall be less than 1, preferable as low as possible.    -   3. Fixate the disk in the bottom of the container, eg        compressing the wall of the container.    -   4. Ad a lid and create a vacuum inside the container    -   5. Insert needle in the patient    -   6. Connect the needle to the container without losing the vacuum    -   7. Draw blood into a plastic container by the help of the        vacuum.    -   8. Spin the tube at 3000 g for 8 min. At this stage the        leucocytes will be on top of the red blood cells and the fibrin        will be polymerized through the upper serum layer as the g force        is low and not able to compress it on top of the platelets.    -   9. Release the disk in the bottom    -   10. Spin the tube at 3000 g for 2 min. This will cause the disk        to move to the top and thereby collecting the leukocytes and        platelets and compress the fibrin layer into one sheet.    -   11. Remove lid and remove the blood product, that is placed in        top of the contain

Example 5

-   -   1. Take a 20 ml container (inner diameter: 26 mm) prepared out        of polyamide or polyurethane    -   2. Place a disk in the bottom of the container. The density of        the disk shall be less than 1, preferable as low as possible.    -   3. Fixate the disk in the bottom of the container, eg by        compressing the wall of the container.    -   4. Create a vacuum inside the container and ad a lid    -   5. Insert a needle in the patient    -   6. Connect the needle to the container without losing the vacuum    -   7. Draw blood into a plastic container by the help of the        vacuum,    -   8. Spin the tube at 3700 g for 3 min. At this stage the        leucocytes will be on top of the red cells and the fibrin will        be polymerized through the upper serum layer as the g force is        low and not able to compress it on top of the platelets.    -   9. Wait for 8 minutes.    -   10. Release the disk in the bottom    -   11. Spin the tube at 3000 g for 2 min. This will cause the disk        to move to the top and thereby collecting the leukocytes and        platelets and compress the fibrin layer into one sheet.    -   12. Remove lid and remove the blood product, that is placed in        top of the container

As it appear from the above examples, the combination of coagulationactivation, spin speed (g), spin time, rest time between spin can bevaried within some limits.

These are illustrated on below tables:

Coagulation Coagulation Spin 1. time after or activation speed Spin timeduring 1 spin 2. Spin Low Low Long Long Yes, high Low Low Long Long Yes,can be low if fibrin adhesion to container wall is mechanical releasedfrom wall or adheasion to the wall is low. Low High Short Long Yes, highHigh High Long Short No High High Short Short Yes, high

If processing with a disk:

Coagulation Coagulation Spin time after 2. Spin were the activationspeed 1. Spin time or during 1 spin disk is released Low Low Long LongLow Low High Short Long Low High High Long Short Low High High ShortShort Low

Example 6 Optimization of Relative Centrifugation Force and Time

-   -   1. Full blood was drawn into 6 ml EDTA tubes (Vacutainer, BD®).    -   2. 20 ml container (inner diameter: 26 mm) prepared out of        polyamide or polyurethane filled with 18 ml and spun at        different RCFs for different times    -   3. Samples (˜300 μl) were taken by a syringe at the bottom        (approx 5 mm above the bottom) and top (approx 5 mm below the        surface) after the above spin times—afterwards the spin was        continued to obtain the next sample. Bottom samples were diluted        1:1 with D-PBS.    -   4. Samples were analyzed by automated cell counting (XE 2100,        Sysmex Corporation) and cell numbers in the original sample        calculated. Results are given in millions of cells per ml.

Millions of platelets per milliliter in the upper (top) and lower(bottom) part of blood centrifuged at the given relative centrifugationforce (g) as a function of time (min):

Minutes 0 1 3 5 7 11 2000 g top 178 480 224 113 59 13 2000 g bottom 1787 5 3 2 4 3000 g top 178 378 103 38 14 0 3000 g bottom 178 3 2 5 3 13700 g top 178 364 97 27 8 0 3700 g bottom 178 2 11 2 1 0

Millions of Leucocytes per milliliter in the upper (top) and lower(bottom) part of blood centrifuged at the given relative centrifugationforce (xg) as a function of time (min):

Minutes 0 1 3 5 7 11 2000 g 7.43 0.28 0 0 0 0 top 2000 g 7.43 0.89 0.020.13 0.26 0.12 bottom 3000 g 7.43 0.19 0 0 0.01 0 top 3000 g 7.43 0.070.04 0.11 0.02 0.02 bottom 3700 xg 7.43 0.05 0.03 0 0 0 top 3700 xg 7.430.03 0.59 0.07 0.02 0.01 bottom

Example 7 Growth Factor Release as a Response to Chronic Wound Fluid

-   -   1. The blood product was generated by the method given in        example 1.    -   2. The blood products was cut in half and placed in 100 μl PBS1%        BSA or 100 μl chronic wound fluid (collected over 24 hrs from a        venous leg ulcer) and incubated at 37 degrees celcius.    -   3. After given time points (1, 2, 3.5, 7, 14, 22 and 29 hours)        the samples were spun at 16000 g for 10 min, and the supernatant        transferred to a new tube, added 1/10 th (81 μl sample+9 μl PI)        Protease Inhibitor (Complete®, Roche) and frozen at −80 degree        celcius.    -   4. Platelet derived growth factor—AB levels in were determined        by using an ELISA kit (DuoSet® ELISA cat. No. DY222, R&D        systems) as described by the manufacturer. PDGF-AB        concentrations in the original samples were calculated.

Platelet derived growth factor AB (PDGF-AB) release from blood product(ng/ml blood product) as a function of time (hrs).

Time (hours) 1 2 4 7 22 29 Chronic Wound fluid (control) 0 0 0 0 0 0Blood product in PBS 153 172 160 174 206 233 Blood product in chronic426 490 602 497 234 275 wound fluid

Example 8

-   -   1. The blood product was generated by the method given in        example 1.    -   2. Two blood products were incubated in 1 ml DMEM (PAA, Germany)        at 37 C and 5% CO2 for 48 hrs.    -   3. In parallel 2 blood products were incubated in 1 ml DMEM        (PAA, Germany) including lipopolysaccharide ((10 ng/ml) (LPS        derived from Escherichia coli; L2654; Sigma-Aldrich) at 37 C and        5% CO2 for 48 hrs.    -   4. After 48 hrs the media were transferred to microcentrifuge        tubes and spun 20 min at 16200×g. The supernatants were frozen        at −80 C until analysis.    -   5. Proteome profiler Arrays ARY007 and ARY005 (both R&D systems)        were performed as described by R&D systems, except that buffer 4        (ARY007) were used in both kits. 420 ul supernatant were diluted        in 500 ul buffer 4 and 580 ul buffer 5 as described by R&D        systems.    -   6. Reactivity with arrays were detected using chemiluminescent        HRP substrate (Immobilon Western™, Millipore, US),    -   7. Light emission were captured using a Fluorchem 3000 system        (Alpha Innotech. US). Mean pixel density were extracted by the        Fluorchem software (Alpha Innotech, US).

Blood product + Blood product Lipopolysaccharide Substance detected(Mean pixel density) (Mean pixel density) CXCL8 (IL-8) 2605 404 CXCL 10(IP-10) 305.5 48.5 MMP-8 518 214 IL-1ra 1825.5 1117.5 L-16 171 105 MMP-92663.5 1729.5 Angiopoietin-1 676.5 537.5 PDGF-AB/PDGF-BB 851.5 704.5PDGF-AA 1357 1159.5 CXCL16 300 256.5 TIMP-1 2507.5 2170.5 Endostatin 187175.5 Angiogenin 689 650.5 MIF 1989 1880.5 IGFBP-2 1942 1883.5 IGFBP-3444 468 EGF 612.5 670.5 IGFBP-1 291.5 401 sICAM-1 635.5 894.5 PAI-1 19402897.5 CCL5 (RANTES) 4104 6151.5 CD26 458.5 828.5 VEGF 246.5 891.5 CXCL1(GRO-alpha) 336 2236 CCL4 (MIP-1-beta) 7 117.5 CCL2 (MCP-1) 6.5 334G-CSF 7.5 429.5 IL-1Beta 7 600 IL-6 8 2094.5

The invention claimed is:
 1. A blood product (10) comprising: componentsfrom whole blood, including fibrin, thrombocytes and leukocytes; theblood product (10) comprising: a first outer surface, a second outersurface, a first layer (21), a second layer (22) and a third layer (23);the second layer (22) being adjacent to the first layer (21) and thethird layer (23); the first layer (21) defining the first outer surface(24) of the blood product (10); the third layer (23) defining the secondouter surface (25) of the blood product (10); wherein a majority of thefirst layer (21) by volume and/or mass comprises fibrin; a majority ofthe second layer (22) by volume and/or mass comprises thrombocytes; anda majority of the third layer (23) by volume and/or mass comprisesleukocytes; and wherein the first layer (21), the second layer (22), andthe third layer (23) are substantially parallel to each other.
 2. Theblood product according to claim 1, wherein a majority of the fibrinpresent in the blood product (10) is present in the first layer (21). 3.The blood product according to claim 1, wherein a majority of thethrombocytes present in the blood product (10) are present in the secondlayer (22).
 4. The blood product according to claim 1, wherein amajority of the leukocytes present in the blood product (10) are presentin the third layer (23).
 5. The blood product according to claim 1,wherein the blood product (10) solely consists of components from wholeblood.
 6. The blood product according to claim 1, wherein the bloodproduct (10) further comprises a first substance chosen from a groupconsisting of fibroblasts, keratinocyte cells and hyaluronic acid.